AcidPhenolYeastRNAPrep
This is the preferred method for yeast RNA preparationuse Gloves and RNAse free solutions throughout.1. Use a YPD overnight culture to innoculate fresh YPD media and grow cells at 30 degrees overnight. Example: 120 microliters O/N in 800 ml YPD gives A600 ~0.85 after ~16 hrs.2. For RNA samples from exponentially growing cells, take samples between A600 0.5 – 1.0. Remove the equivalent of 200 ml of A600 ~1.0 cell......閱讀全文
Acid-Phenol-Yeast-RNA-Prep
This is the preferred method for yeast RNA preparationuse Gloves and RNAse free solutions throughout.1. Use a YPD overnight culture to innoculate fres
Yeast-DNA-Prep
Protocolgrow up yeast culture to appropriate density (near saturation)spin 1.5 mls of culture for 1 min in microfuge and aspirate off supernatantresus
Yeast-Genomic-DNA-Prep
Grow 10ml YPD cultures o/n. Figure out cell density; inoculate 30 ml YPD and grow o/n so that cell density is approximately 2 x 108cells/ml the next m
酵母準備
Yeast DNA PreparationYeast Genomic Preparation? (Gottschling Lab)Rapid method for yeast genomic DNA isolation??Yeast DNA Preparation (rapid glass bead
Quick-Yeast-DNA-Prep:-Isolation-of-Total-DNA-(genomic-and-plasmid)
Grow a 5 ml YPD O/N culture inoculated with a single yeast colony at 30 deg.Transfer culture to a small 13 x 100 glass tube. Spin down cells 2 min. in
Invitro-Phagocytosis-Assay-of-Macrophages
IntroductionThe term phagocytosis itself describes its mean phage = engulfment; cytosis: cell process. In other words, phagocytosis is the cellular pr
RNA-extraction-using-trizol/tri
RNA extraction with TRIzol (Invitrogen product name) or the equivalent TRI (Sigma-Aldrich product name) is a common method of total?RNA extraction?fro
A-quick-RNA-miniprep-for-Neurospora-mycelial-cultures
Most RNA isolation techniques currently in use have been developed for the processing of large quantities of material. These typically involve multipl
General-Laboratory-Procedures,-Equipment-Use,-and-Safety-Considerations
A. Storage .The following properties of reagents and conditions are important considerations in processing and storing DNA and RNA. Heavy metals promo
Phenol/chloroform-extraction
General InformationPhenol/chloroform extraction is an easy way to remove proteins from your nucleic acid samples and can be carried out in a manner th
質粒的小量制備
·?????????Standard (alkaline lysis) Mini-Prep?(Goldberg Lab)Standard protocol for mini-prep and recipe for solution I, II and III.Alkaline Lysis Minip
質粒的小量制備
·?????????Standard (alkaline lysis) Mini-Prep?(Goldberg Lab)Standard protocol for mini-prep and recipe for solution I, II and III.Alkaline Lysis Minip
Fast-and-reliable-miniprep-RNA-extraction-from-Neurospora-crassa
We have developed a method for isolating high quality total RNA from?N. crassa?mycelia that reliably yields large quantities. It is possible to extrac
RNA-Extraction-(mini-prep):Trizol法實驗原理和步驟
RNA的制備與分析對于了解基因在轉錄水平上的表達與調控和cDNA的合成都是必須的,RNA的純度和完整性對于Northern blot,RT-PCR 和cDNA文庫的構建等分子生物學實驗都至關重要。RNA分離的方法很多,其中最關鍵的因素是盡量減少RNA酶的污染 實驗原理: ?Trizol 試劑
E.Z.N.A.TM-Yeast-RNA-Kit-Spin-Protocol
實驗概要The E.Z.N.A.? Yeast RNA Kit allows convenient isolation of high-quality total RNA from a wide variety of yeast species. Up to 2 x 107 log-phase cu
ISOLATION-OF-RNA-FROM-BACTEROIDS
3 g nodules (fresh or frozen in liquid N2) were ground to a powder in mortar and pestle with liquid N2. To the powder was added ice cold 0.5 M mannito
細菌的核酸抽提
DNA Extraction·?????????DNA Extraction from Bacteria?(Julie B. Wolf,UMBC)Phenol/chloroform method·?????????DNA Extraction From Bacteria (Triton Method
Genomic-DNA-Extraction--Phenol-|-Chloroform
實驗概要This section provides a general protocol for genomic DNA extraction using phenol and chloroform.主要試劑1.?????? Glycogen (20 μg/μL)2.?????? 7.5 M NH4
TRIzol-Prep
Procedure1.? Homogenize cells (10 million) or tissue (50-100 mg) in 1 mL?TRIzol Reagent?(e.g. scrape and pass through 30G needle, dounce homogenize an
RNA提取
RNA提取(主要內容如下)Tips for Handing RNA?Total RNA IsolationmRNA IsolationrRNA IsolationOthersQ & A posted in the Method Forum??Basic Procedures for Handing
Sauer:RNA-Purification-from-E.-coli
My Experience Purifying RNA from E. coliRegarding RNA extraction, there is a horrible tendency of people to use kits for RNA extraction with bacteria.
Yeast-Media
YEPD (non-selection)-1% yeast extract-2% peptone-1.5% agar (if needed for plates)After autoclaving add glucose to 2% by adding 100 ml of 20% solution
Isolation-of-microRNA-(miRNA)
實驗概要? ? ? ? This protocol utilizes the powerful guanidine isothiocyanate–phenol:chloroform extraction method which allows the rapid isolation of t
蛋白質提取和純化
蛋白質提取和純化(主要內容如下)Protein Extraction?Protein PurificationProtein PrecipitationColumn PreparatioinQ & A Posted in the Method ForumProtein ExtractionWhole
CHO-Centrosome-Prep
CHO Centrosome Prep:Arshad Desai4/94Cells:We grow our CHOs with MEM[[alpha]] (without nucleosides) + 10% Bovine Calf Serum and penn/strep/glutamine. F
Studier-Lysate-Prep
SummaryHow to make a lysate from a plaque preparation. We also use this protocol for preparation of a quick stock from previously made lysate prep.Pro
Neutralizing-Arachidonic-Acid
NOTE - Use arachidonic acid from Biomol (# FA-003)1) Make up the appropriate concentration of AA in 100% ethanol.2) Add 1μl of phenol red solution.-->
The-Citric-Acid-Cycle
The Krebs cycle, also called the citric acid cycle, is a fundamental metabolic pathway involving eight enzymes essential for energy production through
Amino-acid-composition
There has been a recent revival of interest in the use of AA composition for the identification of proteins from 2-D gels. This technique uses the idi
Arachidonic-Acid-Labeling
1) Grow cells to a density of 5-8 X 105 cells/ml in RPMI 1640 containing serum.2) Pellet cells and wash 1 time with room temperature PBS.3) Resuspend